Determination of carbendazim, fuberidazole and thiabendazole by three-dimensional excitation-emission matrix fluorescence and parallel factor analysis

We simultaneously determined carbendazim, fuberidazole and thiabendazole by excitation-emission matrix (EEM) fluorescence in combination with parallel factor analysis (PARAFAC). Three-way deconvolution provided the pure analyte spectra from which we estimated the selectivity and sensitivity of the pesticides, and the relative concentration in the mixtures from which we established a linear calibration. Special attention was given calculating such figures of merit as precision, sensitivity and limit of detection (LOD), derived from the univariate calibration curve. The method, which had a relative precision of around 2-3% for the three pesticides, provided limits of detection of 20 ng ml⁻¹ for carbendazim, 4.7 ng ml⁻¹ for thiabendazole and 0.15 ng ml⁻¹ for fuberidazole. The accuracy of the method, evaluated through the root mean square error of prediction (RMSEP), was 27.5, 1.4, and 0.03 ng ml⁻¹, respectively, for each of the pesticides.     

Determination of phenol in the presence of its principal degradation products in water during a TiO2-photocatalytic degradation process by three-dimensional excitation-emission matrix fluorescence and parallel factor analysis

This paper describes a simple and rapid way of monitoring a photocatalytic degradation of phenol in aqueous suspensions of TiO₂. A three-way analytical methodology based on fluorescence excitation-emission matrix (EEM) and parallel factor analysis (PARAFAC) was developed to resolve the species present in the reaction mixture and quantify the concentration of phenol and its principal degradation products throughout the degradation. Parameters such as core consistency, fit% and correlation coefficients between recovered and pure spectra were used to determine the appropriate number of factors for the PARAFAC model. The accuracy of the model was evaluated by the root mean square error of prediction (RMSEP). Using a four-factors PARAFAC model, phenol, hydroquinone, resorcinol and catechol, were satisfactorily determined. The proposed method is an interesting alternative to the traditional techniques normally used for monitoring degradation reactions.     

Second-order calibration of excitation-emission matrix fluorescence spectra for determination of glutathione in human plasma

A rapid non-separative spectroflourimetric method based on the second-order calibration of the excitation-emission data matrix was proposed for the determination of glutathione (GSH) in human plasma. In the phosphate buffer solution of pH 8.0 GSH reacts with ortho-phthaldehyde (OPA) to yield a fluorescent adduct with maximum fluorescence intensity at about 420 nm. To handle the interfering effects of the OPA adducts with aminothiols other than GSH in plasma as well as intrinsic fluorescence of human plasma, parallel factor (PARAFAC) analysis as an efficient three-way calibration method was employed. In addition, to model the indirect interfering effect of the plasma matrix, PARAFAC was coupled with standard addition method. The two-component PARAFAC modeling of the excitation-emission matrix fluorescence spectra accurately resolved the excitation and emission spectra of GSH, plasma (or plasma constituents). The concentration-related PARAFAC score of GSH represented a linear correlation with the concentration of added GSH, similar to that is obtained in simple standard addition method. Using this standard addition curve, the GSH level in plasma was found to be 6.10 ± 1.37 μmol L⁻¹. The accuracy of the method was investigated by analysis of the plasma samples spiked with 1.0 μmol L⁻¹ of GSH and a recovery of 97.5% was obtained.     

Interference-free determination of fluoroquinolone antibiotics in plasma by using excitation-emission matrix fluorescence coupled with second-order calibration algorithms

Fluoroquinolones or so-called second-generation quinolones, in particular, ofloxacin (OFL), norfloxacin (NOR), and enoxacin (ENO), with therapeutic advantages possess strongly overlapped fluorescence spectra. In this paper, two strategies were proposed for simultaneous direct determination of OFL, NOR and ENO in plasma by combining fluorescence excitation-emission matrix (EEM) with second-order calibration based on the alternating trilinear decomposition algorithm (ATLD) and parallel factor analysis (PARAFAC). The results showed that both algorithms could solve the problem of serious fluorescence spectral overlapping of the sought-for analytes even in the presence of uncalibrated interferents. However, ATLD has advantages of being insensitive to overestimated component number and fast convergence. The results by using ATLD with an estimated component number of five were reasonably acceptable for clinical analysis. The average recoveries of OFL, NOR and ENO in synthetic samples were 99.7 ± 2.4, 101.5 ± 2.4 and 97.3 ± 3.8%, respectively; the average recoveries of OFL, NOR and ENO in complex plasma were 94.3 ± 2.6, 85.6 ± 3.3 and 103.3 ± 3.0%, respectively.     

Rapid analysis of anthracycline antibiotics doxorubicin and daunorubicin by microchip capillary electrophoresis

A simple and rapid method has been developed for the analysis of anthracycline antibiotics doxorubicin (DOX) and daunorubicin (DAU) in human serum using mirochip-based capillary electrophoresis (CE) with laser-induced fluorescence (LIF) detection. In this study, method development included studies of the effect of buffer pH, buffer concentration, organic solvents and separation voltage on sensitivity and separation efficiencies for the CE separation of DOX and DAU. Acetonitrile was found to have significantly improved the sensitivity and separation efficiency. The method was validated with regard to reproducibilities, linearity and limit of detection (LOD). The optimum electrophoretic separation conditions were 10 mM sodium tetraborate buffer at pH 9.5 with 40% acetonitrile (V/V) and a separation voltage of 2.1 kV. DOX and DAU were separated in 60 s under the optimum separation conditions. Linear relationships were obtained between the concentration and peak area (or peak height) in the 1–75 µg mL^{− 1} range and with the detection limits of 0.3 and 0.2 μg mL^{− 1} for DOX and DAU, respectively. The stability of both migration time and peak height of the analytes showed relative standard deviations of less than 5% (n = 9). The potential of this method was verified by spiking a human serum sample with the two drugs and analyzing the recovery ratios.     

The maintenance of the second-order advantage: second-order calibration of excitation-emission matrix fluorescence for quantitative analysis of herbicide napropamide in various environmental samples

A rapid non-separative spectrofluorometric method based on the second-order calibration of excitation-emission matrix (EEM) fluorescence was proposed for the determination of napropamide (NAP) in soil, river sediment, and wastewater as well as river water samples. With 0.10 mol L⁻¹ sodium citrate-hydrochloric acid (HCl) buffer solution of pH 2.2, the system of NAP has a large increase in fluorescence intensity. To handle the intrinsic fluorescence interferences of environmental samples, the alternating penalty trilinear decomposition (APTLD) algorithm as an efficient second-order calibration method was employed. Satisfactory results have been achieved for NAP in complex environmental samples. The limit of detection obtained for NAP in soil, river sediment, wastewater and river water samples were 0.80, 0.24, 0.12, 0.071 ng mL⁻¹, respectively. Furthermore, in order to fully investigate the performance of second-order calibration method, we test the second-order calibration method using different calibration approaches including the single matrix model, the intra-day various matrices model and the global model based on the APTLD algorithm with nature environmental datasets. The results showed the second-order calibration methods also enable one or more analyte(s) of interest to be determined simultaneously in the samples with various types of matrices. The maintenance of second-order advantage has been demonstrated in simultaneous determinations of the analyte of interests in the environmental samples of various matrices.     

Correction of inner-filter effect in fluorescence excitation-emission matrix spectrometry using Raman scatter

Fluorescence excitation-emission matrix (EEM) spectroscopy is a useful tool for interpretation of fluorescence information from natural water samples. One of the major problems with this technique is the inner-filter effect (IFE), i.e. absorption of light at both the excitation and emission wavelengths. The common solutions are to either dilute the sample or apply some form of mathematical correction, most often based on the measured absorbance of the sample. Since dilution is not always possible, e.g. in on-line or in situ EEM recordings, and corrections based on absorbance are hampered primarily by the use of a separate absorbance instrument, neither of these solutions is optimal. In this work, we propose a mathematical correction procedure based on the intensity of Raman scatter from water. This procedure was found to reduce the error after correction by up to 50% in comparison with two absorbance correction procedures. Furthermore, it does not require the use of a separate absorbance measurement, and it is applicable to on-line and in situ EEM recordings, where the IFE would otherwise cause problems.     

Quantitative analysis of hydrolysis of carbaryl in tap water and river by excitation-emission matrix fluorescence coupled with second-order calibration

A novel method was proposed to determine simultaneously carbaryl and its degradation product 1-naphthol in river and tap water in this paper. The parallel factor analysis (PARAFAC) algorithm was adopted to analyze the excitation–emission matrix (EEM) fluorescence data. The second-order advantage of the PARAFAC-based second-order calibration algorithm was exploited, which make it possible that calibration can be performed even in the presence of unknown interferences. Good recoveries were obtained although the excitation and emission spectral profiles of the analytes were overlapped with background in the river water. It was also applied to investigate the hydrolysis kinetics of carbaryl in river water and tap water. The rate equation, the rate constant and the half life were calculated.     

交替三线性分解算法用于水杨酸和2,5-二羟基苯甲酸的荧光法同时测定

水杨酸 (SA)、2 ,5 二羟基苯甲酸 (GA)和对 氨基苯甲酸 (PABA)的荧光光谱相互重叠。用交替三线性分解二阶校正法对PABA共存下的SA和GA进行了同时荧光测定 ,SA和GA的回收率分别为 (1 0 1 2± 1 9) %和 (97 1 6±1 0 4 ) %。     

Application of multi-way data analysis on excitation-emission spectra for plant identification

The ability to distinguish among diets fed to Damascus goats using excitation-emission luminescence spectra was investigated. These diets consisted of Medicago sativa L. (alfalfa), Trifolium spp. (clover), Pistacia lentiscus, Phyllirea latifolia and Pinus brutia. The three-dimensional luminescence response surface from phosphate buffered saline (PBS) extracts of each material was analyzed using muti-way analysis chemometric tools (MPCA) and parallel factor analysis (PARAFAC). Using three principal components, the spectra from each diet material were distinguished. Additionally, fecal samples from goats fed diets of either alfalfa or clover hays were investigated. The application of MPCA and PARAFAC to these samples using models derived from the pre-digested diet materials was strongly suggestive of the utility of similarly derive training samples for the elucidation of botanical diet composition for animals.     

Simultaneous analysis of the photocatalytic degradation of polycyclic aromatic hydrocarbons using three-dimensional excitation-emission matrix fluorescence and parallel factor analysis

Polycyclic aromatic hydrocarbons (PAHs) may be photochemically degraded. Monitoring of degradation process of PAHs is carried out by traditional methods, which normally imply time-consuming procedures that do not allow the chemical process to be analyzed in real time. In the present study, photodegradation kinetics of dibenz[a,h]anthracene, benz[a]anthracene, benz[a]pyrene and benz[k]fluorantene were investigated in aqueous solutions under different conditions. A 2³ factorial design was used for optimizing the degradation process.Fluorescence spectroscopy is a fast, cheap and sensitive analytical method, attractive for use in conjunction with chemometric methods; in this case three-way analytical methodology based on fluorescence excitation-emission matrix (EEM) and parallel factor analysis (PARAFAC) was employed. A four-factor PARAFAC model made it possible to resolve the species presents in the degradation mixture and quantify the relative concentration of the analytes throughout the degradation. Several different parameters, such as core consistency, percentage of fit and correlation coefficients between recovered and reference spectra were employed to determine the suitable number of factors for the PARAFAC model. This new methodology allows us to determine satisfactorily the PAHs concentration during the photodegradation in mixtures of arbitrary composition, representing an interesting alternative to the conventional techniques normally used for the monitoring of degradation reactions.     

Application of unfold principal component analysis and parallel factor analysis to the exploratory analysis of olive oils by means of excitation-emission matrix fluorescence spectroscopy

Discrimination between virgin olive oils and pure olive oils is of primary importance for controlling adulterations. Here, we show the potential usefulness of two multiway methods, unfold principal component analysis (U-PCA) and parallel factor analysis (PARAFAC), for the exploratory analysis of the two types of oils. We applied both methods to the excitation-emission fluorescence matrices (EEM) of olive oils and then compared the results with the ones obtained by multivariate principal component analysis (PCA) based on a fluorescence spectrum recorded at only one excitation wavelength. For U-PCA and PARAFAC, the ranges studied were λ_ex=300-400 nm, λ_em=400-695 nm and λ_ex=300-400 nm, λ_em=400-600 nm. The first range contained chlorophylls, whose peak was much more intense than those of the rest of species. The second range did not contain the chlorophylls peak but only the fluorescence spectra of the remaining compounds (oxidation products and Vitamin E). The three-component PARAFAC model on the second range was found to be the most interpretable. With this model, we could distinguish well between the two groups of oils and we could find the underlying fluorescent spectra of three families of compounds.     

Determination of daunomycin in human plasma and urine by using an interference-free analysis of excitation-emission matrix fluorescence data with second-order calibration.

Daunorubicin (DNR) is a significant antineoplastic antibiotic, which is usually applied to a chemotherapy of acute lymphatic and myelogenous leukaemia. Unfortunately, cardiotoxicity research in animals has indicated that DNR is cardiotoxic. Therefore, it is important to quantify DNR in biological fluids. A new algorithm, the alternating fitting residue (AFR) method, and the traditional parallel factor analysis (PARAFAC) have been utilized to directly determine DNR in human plasma and urine. These methodologies fully exploit the second-order advantage of the employed three-way fluorescence data, allowing the analyte concentrations to be quantified even in the presence of unknown fluorescent interferents. Furthermore, in contrast to PARAFAC, more satisfactory results were gained with AFR.     

Simultaneous determination of 6-methylcoumarin and 7-methoxycoumarin in cosmetics using three-dimensional excitation-emission matrix fluorescence coupled with second-order calibration methods

This paper reports a simple, rapid, and effective method for quantitative analysis of 6-methylcoumarin (6-MC) and 7-methoxycoumarin (7-MOC) in cosmetics using excitation–emission matrix (EEM) fluorescence coupled with second-order calibration. After simple pretreatments, the adopted calibration algorithms exploiting the second-order advantage, i.e., parallel factor analysis (PARAFAC) and self-weighted alternating tri-linear decomposition (SWATLD), could allow the individual concentrations of the analytes of interest to be predicted even in the presence of uncalibrated interferences. In the analysis of facial spray, with the external calibration method, the average recoveries attained from PARAFAC and SWATLD with the factor number of 3 (N = 3) were 101.4 ± 5.5 and 97.5 ± 4.1% for 6-MC, and 103.3 ± 1.7 and 101.7 ± 1.8% for 7-MOC, respectively. Moreover, in the analysis of oil control nourishing toner, the standard addition method (SAM) was suggested to overcome the partial fluorescence quenching of 6-MC induced by the analyte–background interaction, which also yielded satisfactory prediction results. In addition, the accuracy of the two algorithms was also evaluated through elliptical joint confidence region (EJCR) tests as well as figures of merit (FOM), including sensitivity (SEN), selectivity (SEL) and limit of detection (LOD). It was found that both algorithms could give accurate results, only the performance of SWATLD was slightly better than that of PARAFAC in the cases suffering from matrix effects. The method proposed lights a new avenue to determine quantitatively 6-MC and 7-MOC in cosmetics, and may hold great potential to be extended as a promising alternative for more practical applications in cosmetic quality control, due to its advantages of easy sample pretreatment, non-toxic and non-destructive analysis, and accurate spectral resolution and concentration prediction.     

三维荧光光谱二阶校正方法测定血浆样中喷昔洛韦及泛昔洛韦含量

利用三维荧光光谱即激发发射矩阵荧光光谱与化学计量学的基于平行因子分析(PARAFAC)算法的二阶校正方法相结合,尝试对血浆样中泛昔洛韦及其活性代谢物喷昔洛韦的含量进行同时定量测定.当算法选取组分数为3时,解析得到血浆样中泛昔洛韦和喷昔洛韦的平均回收率分别为(102.4±3.4)%和(105.1±2.3)%.结果表明该分析策略可准确可靠地实现血浆样中泛昔洛韦和喷昔洛韦的直接同时快速定量测定.     

Determination of cisapride in human plasma by high-performance liquid chromatography with fluorescence detection

Summary A new sensitive HPLC-FLD method has been developed and validated for the determination of cisapride in human plasma for a bioequivalence study. A gradient method was used to remove late-eluting plasma components of no interest. The separation was performed on a Li-ChroCART 250-4 Purospher RP-18 (5 μm particle) analytical column fitted with a LiChroCART 4-4 Purospher RP-18 endcapped (5 μm particle) guard column. The excitation and emission wavelengths were 295 and 350 nm during fluorescence detection. The calibration plot was linear in the range of 5–200 ng mL⁻¹. A demethoxy analogue of cisapride was used as internal standard.     

Determination of Riboflavin in Human Plasma by Excitation‐Emission Matrix Fluorescence and Multi‐Way Analysis

Direct determination of riboflavin (Fig. 1), a vitamin, in human plasma was accomplished based on excitation‐emission matrix (EEM) fluorescence measurements and multi‐way chemometrics method based on parallel factor analysis (PARAFAC). The PARAFAC trilinear model, without restrictions and using one factor was used in the data analysis. The excitation wavelength range was from 380 to 460 nm and the emission was recorded from 480 to 600 nm. The calibration set was constructed with sixteen standard solutions in a concentration range of 0.02–0.38 μg mL^?1 for riboflavin. The capabilities of the method for the analysis were evaluated by determination of riboflavin in synthetic and real samples with satisfactory results. The accuracy of the methods, evaluated through the root mean square error of prediction (RMSEP), was 0.0059 for riboflavin by the PARAFAC model. Also, partial least squares (PLS) model was built at one excitation wavelength and used to determine a set of synthetic and real samples. The best model was obtained with PARAFAC. This result shows that molecular fluorescence spectroscopy can be used for the development of robust analytical methods for the direct determination of riboflavin in complex backgrounds such as human plasma.     

Simultaneous determination of tyrosine and dopamine in urine samples using excitation-emission matrix fluorescence coupled with second-order calibration

A "green" and quick analytical method for complex compounds was developed for simultaneous determination of tyrosine (Tyr) and dopamine (DA) in urine samples in this paper. The three-way responsive data recorded by excitation-emission matrix fluorescence (EEM) spectrometer was analyzed using second-order calibration methods based on both parallel factor analysis (PARAFAC) and selfweighted alternating trilinear decomposition (SWATLD) algorithms. The EEM spectra of the analytes were overlapped with the background in urine samples. However the second-order advantage of both PARAFAC and SWATLD methods was exploited, even in the presence of unknown interferences and the satisfactory results can be obtained. Furthermore, the linear ranges of Tyr and DA were determined to be 0.042-6.42 μg/mL and 0.18-4.43 μmg/mL, respectively, and the accuracies of both methods were validated by the analytical figures of merit (FOM).     

Simultaneous determination of naphazoline and pyridoxine in eye drops using excitation–emission matrix fluorescence coupled with second-order calibration method based on alternating trilinear decomposition algorithm

A novel method is developed for the direct determination of naphazoline hydrochloride(NAP) and pyridoxine hydrochloride(VB6) in commercial eye drops. By using excitation–emission matrix(EEM)fluorescence coupled with second-order calibration method based on the alternating trilinear decomposition(ATLD) algorithm, the proposed approach can achieve quantitative analysis successfully even in the presence of unknown and uncalibrated interferences. The method shows good linearity for NAP and VB6 with correlation coefficients greater than 0.99. The results were in good agreement with the labeled contents. To further confirm the feasibility and reliability of the proposed method, the same batch samples were analyzed by multiple reaction monitoring(MRM) based on LC–MS/MS method.T-test demonstrated that there are no significant differences between the prediction results of the two methods. The satisfactory results obtained in this work indicate that the use of the second-order calibration method coupled with the EEM is a promising tool for industrial quality control and pharmaceutical analysis due to its advantages of high sensitivity, low-cost and simple implementation.     

Highly sensitive fluorescence quantification of irinotecan in biological fluids with the aid of second-order advantage

<正>A rapid,green and highly sensitive excitation-emission matrix(EEM) fluorescence method was proposed for analysis of irinotecan(CPT-11) in biological fluids including human plasma and urine samples of uncalibrated interferences with the aid of second-order advantage.Due to the serious spectral overlapping from biological matrices,the parallel factor analysis(PARAFAC) and the alternating normalization-weighted error(ANWE) have been recommended to perform directly calibration and overcome the problem which makes the traditional fluorospectrophotometer in trouble.Satisfactory results can be achieved.Furthermore, performance of the proposed method was evaluated based on figures of merit and some statistical parameters.The accuracy of both algorithms was validated by the elliptical joint confidence region(EJCR) test.The precision and repeatability were also investigated by the relative standard deviations(RSDs) of intra-day and inter-day.